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首页> 外文期刊>Molecular and Cellular Biology >MOF and H4 K16 Acetylation Play Important Roles in DNA Damage Repair by Modulating Recruitment of DNA Damage Repair Protein Mdc1
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MOF and H4 K16 Acetylation Play Important Roles in DNA Damage Repair by Modulating Recruitment of DNA Damage Repair Protein Mdc1

机译:MOF和H4 K16乙酰化通过调节DNA损伤修复蛋白Mdc1的募集在DNA损伤修复中发挥重要作用

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MOF (MYST1) is the major enzyme to catalyze acetylation of histone H4 lysine 16 (K16) and is highly conserved through evolution. Using a conditional knockout mouse model and the derived mouse embryonic fibroblast cell lines, we showed that loss of Mof led to a global reduction of H4 K16 acetylation, severe G2/M cell cycle arrest, massive chromosome aberration, and defects in ionizing radiation-induced DNA damage repair. We further showed that although early DNA damage sensing and signaling by ATM were normal in Mof-null cells, the recruitment of repair mediator protein Mdc1 and its downstream signaling proteins 53bp1 and Brca1 to DNA damage foci was completely abolished. Mechanistic studies suggested that Mof-mediated H4 K16 acetylation and an intact acidic pocket on H2A.X were essential for the recruitment of Mdc1. Removal of Mof and its associated proteins phenocopied a charge-neutralizing mutant of H2A.X. Given the well-characterized H4-H2A trans interactions in regulating higher-order chromatin structure, our study revealed a novel chromatin-based mechanism that regulates the DNA damage repair process.
机译:MOF(MYST1)是催化组蛋白H4赖氨酸16(K16)乙酰化的主要酶,并且通过进化高度保守。使用条件基因敲除小鼠模型和衍生的小鼠胚胎成纤维细胞系,我们显示 Mof 的丧失导致H4 K16乙酰化的整体降低,严重的G 2 / M细胞周期停滞,大量染色体畸变以及电离辐射诱导的DNA损伤修复中的缺陷。我们进一步表明,尽管在 Mof -null细胞中,通过ATM进行的早期DNA损伤感测和信号转导是正常的,但完全消除了修复介体蛋白Mdc1及其下游信号蛋白53bp1和Brca1向DNA损伤灶的募集。 。机理研究表明, Mof 介导的H4 K16乙酰化和H2A.X上完整的酸性口袋对Mdc1的募集至关重要。 Mof 及其相关蛋白的去除表型化了H2A.X的电荷中和突变体。考虑到H4-H2A trans 相互作用在调节高级染色质结构中的作用,我们的研究揭示了一种新型的基于染色质的机制,可调节DNA损伤修复过程。

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